用一种新的定量聚合酶链反应方法测定胎鼠和新生鼠肝脏GLUT mRNA

Robert H. Lane , Annette S. Flozak, Rebecca A. Simmons
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引用次数: 29

摘要

葡萄糖转移到肝细胞是由葡萄糖转运蛋白(GLUTs)介导的。GLUT mRNA水平通常通过Northern blot分析测定。逆转录聚合酶链反应(RT-PCR)常用于测量RNA丰度。然而,这种方法只是半定量的,并且在第一链合成过程中没有内部控制。我们设计了一种以牛视紫红质为内对照的共反转录和PCR扩增方法,用于cDNA的合成和扩增。作为该技术验证的一部分,我们确定了视紫红质引物对牛Glut基因没有非特异性扩增,由于扩增的Glut基因的不同区域,扩增效果没有差异,并且没有二级结构效应。我们采用改进的RT-PCR方法检测了GLUT在胎鼠和产后大鼠(第20胎鼠和第d1、d4、d14和d21幼年大鼠幼鼠)肝脏中的表达。随着年龄的增长,GLUT 1 mRNA表达量减少,GLUT 2 mRNA表达量增加。我们能够在胎儿肝脏中检测到少量的GLUT 3,在出生后肝脏中检测到少量的GLUT 5。这种RT-PCR方法提供了一种内部控制,允许在少量组织中测量mRNA水平,使其非常适合用于胎儿和任何mRNA水平低的系统。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Measurement of GLUT mRNA in Liver of Fetal and Neonatal Rats Using a Novel Method of Quantitative Polymerase Chain Reaction

Transfer of glucose into the hepatocyte is mediated by glucose transporters (GLUTs). GLUT mRNA levels are usually measured by Northern blot analysis. Reverse transcription-polymerase chain reaction (RT-PCR) is often used to measure RNA abundance. However, this method is only semiquantitative and has no internal control during first-strand synthesis. We designed a method of coreverse transcription and PCR amplification using bovine rhodopsin as an internal control for both cDNA synthesis and amplification. As part of the validation of this technique, we determined that there was no nonspecific amplification of bovine GLUTs by rhodopsin primers, that there were no differences in amplification due to different regions of the Glut gene amplified, and that there were no secondary structure effects on amplification. We applied our modified method of RT-PCR to measure the ontogeny of GLUT expression in liver of fetal and postnatal rats (d20 fetuses and d1, d4, d14, and d21 juvenile rat pups). GLUT 1 mRNA quantity decreased whereas GLUT 2 increased with age. We were able to detect small quantities of GLUT 3 in fetal liver and of GLUT 5 in postnatal liver. This method of RT-PCR provides an internal control and allows measurement of mRNA levels in small quantities of tissue, making it ideal for use in the fetus and any system in which mRNA levels are low.

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